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CHAPTER 5
PROTEINS
5.1 Introduction
Proteins are complex organic nitrogenous substances found inanimal and plant tissues. The term protein is derived from Greek :Proteios means primary or holding first place.
Protein is the essential constituent of living cells. Protein make upto12% of the protoplasm. They are not only responsible for comprisingthe structure of the cell but are concerned with every function of thecell including those of respiration, catalysis of reactions by enzymes,transport of materials, regulation of metabolism, and defense actions.The foods rich in proteins are known as body building foods.
5.2 Sources of protein
Proteins are obtained from animal and plant sources. The animalsources of proteins include milk, egg, meat, fish, liver etc. Plant sourcesof proteins are pulses, nuts and cereals.
5.3 Amino acids
Amino acids are the simplest units of a protein molecule and theyform the building blocks of protein structure. The general formula of anamino acid can be written as,
C
NH 2
H
COOHR C
NH 2
H
COOHH
R=HG lyc ine
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An amino acid is an amino carboxylic acid. R is the side chain orresidue and it represents the group other than -NH
2 and -COOH. It
may be a hydrogen atom (H) or a methyl group (-CH3) or an aliphatic
group or an aromatic group or a heterocyclic group. The amino acidsare classified based on the nature of R groups.
D and L amino acids
Based on the position of amino group on the asymmetric carbonatom, amino acids exist in two types. They are D and L amino acids.
D form
C NH2
COOH
CH3
CH2N H
HOOC
MirrorL-Form
H3CH
The amino acid having the NH2 group on the right is called
D-amino acid. The amino acid having the NH2 group on the left is
called L-amino acid. These isomers are the mirror images of each other.
All amino acids are α amino acids because the NH2 group is
attached to the α carbon atom which is next to the COOH group.Examination of the structure of an amino acid except glycine, revealsthat the α carbon atom has four different groups attached to it, thusmaking it asymmetric. Because of the presence of asymmetric carbonatom, amino acids exist in two optically active forms, dextrorotatoryand levorotatory.
Dextrorotatory, they rotate plane polarised light in the clockwisedirection. Levorotatory, they rotate plane polarised light in the anticlockwise direction. The direction of optical rotation of an amino acidsindicated by the symbol + and - (+ indicates dextro and - indicatelevo).
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It has been found that L-amino acids are more common than Dforms and most of the naturally occuring amino acids are L-amino acids.Therefore L-amino acids are called natural aminoacids. Since the Lamino acids are more common, the letter “L” is usually omitted, whilerepresenting L-amino acids.
Amino acids are widely distributed in plants and animals.
5.3.1 Properties of amino acids
5.3.1.1 Physical properties
Amino acids are coloureless, crystalline, generally soluble in water,in acid and in alkali but sparingly soluble in organic solvents.
5.3.1.2Chemical properties
i. Ionic forms of amino acids
Amino acids bear atleast two ionizable weak acid groups, a - COOHand a -NH
2. In solution, two forms of these groups, one charged and
another uncharged, exist in protonic equilibrium:
R-COOH R-COO- + H+
R-NH3+ R-NH2 + H+
R-COOH and R-NH3+ represent the protonated or acidic
partners in these equilibria. R-COO- and R-NH2 are the conjugate
bases of the corresponding acids.
ii. Zwitterion
CH3 CH NH3+
COO-
Zwitter ionic structure of alanine
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Due to the presence of an acidic and a basic group in the samemolecule, the amino acid exists largely as a dipolar ion or a zwitterion,which can react as an acid as well as a base. In zwitterion, the protonfrom the carboxylic group is transferred to the amino group. Thus azwitterion carries both positive and negative charges.
In acidic solution an amino acid behave like a protonated derivativeand therefore migrates to the cathode under electric field. In an alkalinemedium, the same amino acid behaves like an anion derivative andtherefore migrates to the anode.
iii. Isoelectric point
The net charge (the algebraic sum of all the positively and negativelycharged groups present) of an amino acid depends upon the pH, orproton concentration of the surrounding medium.
The pH at which an amino acid bears no net charge and hencedoes not migrate to either of the anode or cathode under the influenceof an electric current, is known as the isoelectric point or isoelectricpH.
iv. Reaction with ninhydrin
Ninhydrin oxidatively decarboxylates an amino acid to CO2, NH
3
and an aldehyde. The reduced ninhydrin then reacts with the liberatedammonia forming a purple complex, which absorbs light at a wavelengthof 570 nm.
H+
COO
+
CH COOH
NH3
R OH-
AnionCation Zwitter ion
CH
NH3
+
R CH COO
NH2
R
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OH
OH
O
O
+ NH2 CH COOH
R
OH
H
O
O
+ CO2NH3RCHO
Ninhydrin
Hydrindantin
Amino acid
OH
O
O
+
+ +
OH
H
O
O
+ NH3
O
O
H
O
O
N
Purple complex
Aldehyde
OH
NinhydrinHydrindantin
+ 3H2O
Ammonia
Ammonia
Fig. 5.1 Reaction of an amino acid with ninhydrin
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5.3.2 Classification of amino acids
The amino acids are classified based on the nature of their R groups,in particular their polarity or tendency to interact with water at biologicalpH. The polarity of the R groups varies widely, from totally non polarto highly polar.
5.3.2.1 Non-polar, aliphatic R-group
The R-group in this class of amino acids are non polar (or)hydrophobic. Six amino acids come under this class, which are glycine,alanine, valine, leucine, isoleucine and methionine.
H CH COO-
NH 3+
CH3 CH COO-
NH 3+
GlycineAlanine
CH COO-
NH 3+
Valine
CHCH3
CH3CH COO-
NH 3+
Leucine
CH2
CH3
CH3
CH
CH COO-
NH3+
Isoleucine
CH2
CH3
CH
CH3
CH2 CH COO-
NH3+
Methionine
CH2
S CH3
Glycine has the simplest structure. Methionine is one of the twosulphur containing aminoacids and has a non polar thio ether group inits side chain.
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5.3.2.2 Aromatic R groups
Phenylalanine, tyrosine and tryptophan, with their aromatic sidechains, are relatively non-polar. All can participate in hydrophobicinteractions. The hydroxyl group of tyrosine can form hydrogen bondwith other compounds and it is an important functional group in someenzymes. Tyrosine and tryptophan are significantly more polar thanphenyl alanine because of the hydroxyl group of tyrosine and the nitrogenof the indole ring in tryptophan.
CH2 CH COO-
NH3+
Phenylalanine
CH2 CH COO-
NH3+
HO
Tyrosine
N
H
CH 2 CH COO -
NH 3+
Tryptophan
5.3.2.3 Polar-uncharged R groups
The R groups of these amino acids are more soluble in water ormore hydrophilic, than those of the non polar amino acids because theycontain functional groups that form hydrogen bonds with water. Thisclass of amino acids includes serine, threonine, cysteine, proline,asparagine and glutamine.
The polarity of serine and threonine is contributed by their hydroxylgroups; that of cysteine by its sulphydryl (-SH) group; and that ofasparagine and glutamine by their amide groups. Proline has a distinctcyclic structure and is only moderately polar. Proline has an imino group.Cysteine is readily oxidized to form a covalently linked dimeric amino
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acid called cystine, in which two cysteine molecules are joined by adisulphide bond.
CH2 CH COO-
NH3+
Serine
OH
CH3 CH COO-
NH3+
Threonine
OH
CH CH2 CH COO-
NH3+
Cysteine
SH
CH COO-
NH3+
Asparagine
CH2CH2N
ONH2
+ COO -
Proline
H2N CH COO-
NH3+
Glutamine
CH2C
O
CH2
CH2 CH COO-
NH3+
Cystine
SCH2CH-OOC
NH3+
S
5.3.2.4 Positively charged (basic) R-groups
The most hydrophilic R groups are those that are either positively(-NH
3+) or negatively (-C00-) charged. The amino acids in which the R
groups have significant positive charges at pH 7.0 are lysine, arginineand histidine.
NH3+
Lysine
CH2 CH2 CH2 CH COO-CH2
NH3+
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H
NH3+
Arginine
CH2 CH2 CH2 CH COO-N
C = NH2
NH2
+CH2
NHHN+
CH2 CH COO-
NH 3+
Histidine
5.3.2.5 Negatively charged (Acidic) R groups
The two amino acids having R groups with a net negative charge atpH 7.0 are aspartate and glutamate.
-OOC CH COO-
NH3+
Aspartic acid
CH2
-OOC CH COO-
NH3+
Glutamic acid
CH2 CH2
Based on their inclusion in the diet, amino acids are classified intotwo groups, namely essential amino acids and non-essential amino acids.
5.3.2.6 Essential amino acids
Certain amino acids can not be synthesized by the living organisms.They must be compulsarily included in the diet for normal health.Theseamino acids are called essential amino acids. For human being about10 amino acids are considered as essential.eg,
1. Arginine 6.Methionine
2. Histidine 7. Phenyl alanine
3. Isoleucine 8. Threonine
4. Leucine 9. Tryptophan
5. Lysine 10. Valine
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5.3.2.7 Non-essential amino acids
Certain amino acids can be synthesized in the cells from essentialamino acids or from other compounds. So these amino acids need notbe included in the diet. They are called non-essential amino acids.
5.3.2.8 Non protein amino acids
Certain amino acids which do not exist in proteins are called nonprotein amino acids eg. Ornithine and β-alanine etc..
5.3.2.9 Peptide bonds
In proteins, amino acids are linked together by linkages calledpeptide bonds. The carboxyl group of one amino acid is joined to theα amino group of another amino acid by a peptide bond.
H2N C
H
C
RAmino acid
O
+ C
H
C
Oα α
C
H
C
R Oα
N
H
C
H
R'
C
O
+H2O
Peptide bondAmino acid'
R'
H2NOH H2N OHOH
The peptide bond is also called as the amide bond. The two aminoacids, joined by a peptide bond, constitute a dipeptide. The dipeptideis formed by simple condensation reaction.
The product formed by a peptide bond is called a peptide. Thecompound formed by the linking of three amino acids is called astripeptide. A peptide formed of less than 10 amino acids constitute anoligopeptide. More than 10 amino acids join together to form apolypeptide chain (Fig. 5.2).
HC
C
HN
CH
C
NH
HC
C
HN
CHH 2 N
COOH
R
O
R
O R
O
R
Fig. 5.2 Structure of a polypeptide
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Protein is made up of one or more polypeptide chains
Many proteins, such as myoglobin, consist of a single polypeptidechain. Others contain two or more chains, which may be either identicalor different. For example haemoglobin is formed of 4 polypeptidechains, of which two α chains are of one kind and the other two βchains are of another kind.
N and C terminal ends of protein
An amino acid in a polypeptide is called a residue. A polypeptidehave two ends, namely amino and carboxyl terminal end. The end ofthe polypeptide chain containing amino group is called amino terminalor N-terminal. The end of the polypeptide chain containing carboxylgroup is called carboxyl terminal or C-terminal. The terminal aminoacid with the free amino group is called N-terminal amino acid and theterminal amino acid with the free carboyl group is called C-terminalamino acid.
NH2 CH C NH CH
R1
C
O
NH CH
R2
C NH
O
CH
R4
C OH
N-terminal amino acid C-terminal amino acid
OO
R1, R2,R3 and R4 - Side chains
R3
5.4 Properties of proteins
5.4.1 Physical properties
1. Colour and taste
Proteins are colourless and usually tasteless. These arehomogeneous and crystalline.
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2. Solubility
Solubility of proteins is influenced by pH. Solubility is lowest atisoelectric point and increased with increasing acidity of alkalinity.
3. Optical activity
All protein solutions rotate the plane polarised light to the left i.e.these are levorotatory.
4. Colloidal nature
Because of their giant size, the proteins exhibit many colloidalproperties are:
i. Their diffusion rate is extermely low.
ii. They may produce considerable light-scattering in solution, thusresulting in visible turbidity (Tyndall effect).
5. The comparatively week forces responsible for maintainingsecondary, tertiary and quarternary structure of proteins are readilydistrupted with resulting loss of biologic activity. This distruption of nativestructure is termed denaturation. Physically, denaturation may be viewedas randomizing the conformation of a polypeptide chain without affectingits primary structure (Fig.5.3).
8M urea
Active enzyme(native form)
Inactive enzyme(denatured form)
Fig. 5.3 Denaturation of protein
The biological activity of most proteins is destroyed by exposureto strong mineral acids or bases, heat, urea, acetone, alcohol and ionicdetergents etc. Denatured proteins are less soluble in water.
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5.4.2 Chemical properties
1. Hydrolysis
i. By acidic agents
Proteins upon hydrolysis with concentrated mineral acids suchas, HCl yield amino acids in the form of their hydrochlorides.
ii. By proteolytic enzymes
Under relatively mild conditions of temperature and acidity,certain proteolytic enzymes like pepsin and trypsin hydrolyse theproteins. Enzyme hydrolysis is used for the isolation of certain aminoacids like tryptophan. Two important drawbacks with this type ofhydrolysis are:
a. It requires prolonged incubation and
b. Hydrolysis may be incomplete
2. Colour reaction with Biuret reagent
When a protein solution is treated with alkaline CuSO4 reagent,
the peptide bonds present in the protein interact with copper ions andforms violet coloured Biuret complex (Fig.5.4). The colour deepenswhich depend on the number of peptide bond present in the protein.The sturcture of the voilet complex is
Fig.5.4 Voilet colour complex
All proteins except dipeptides react with Biuret reagent because aminimum of two peptide linkages are involved in this reaction.
NC
HN
C N
O
O
Cu++
N C
NH
CN
O
O
H H
HH
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This reaction is widely used both as a qualitative test for thedetection of proteins and also as a quantitative test for the estimation ofprotein in biological materials.
5.5 Protein structure
The architecture of protein molecule is complex but well organised.To understand this, a clear idea of certain basic details regarding themode of arrangement of the structural units inside the molecule isnecessary. Linder strom - Lang suggest four types of structuralorganisation for proteins. They are
1. Primary structure
2. Secondary structure
3. Tertiary Structure and
4. Quarternary strucutre
5.5.1 Primary structure
The primary structure of protein is defined as the sequence of aminoacid residues making up its polypeptide chain. The protein may beformed of one or more polypeptide chains. The amino acids are arrangedin specific sequence in these polypeptide chain. The amino acid residuesare linked by peptide bonds. The peptide bond is formed between thecarboxyl group of one amino acid and the amino group of adjacentamino acid. Some times the adjacent polypeptide chains are linked bydisulphide bonds.
C
R
C NH C
R
HC
O
NH
O
C
R
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H2N CH C NH
O
CH
R2
C NH
O
CH C
R3
O
NH CH
R4
C
O
OH
N- terminal amino acidC- terminal amino acidPeptide bond
R1
For example the primary structure of a protein can be written as
gly lys leu val ala glu COOHH2N41 2 3 5 6
Each polypeptide chain of any length has at one end a N-terminalamino acid containing free amino group and at the other end a C-terminalamino acid containing a free carboxyl group. The amino acids in apolypeptide chain are numbered from the N-terminal end.
The primary structure has the following salient features
i. Primary structure refers to the linear sequence of amino acidresidues.
ii. The proteins are linear and unfolded
iii. The protein is formed of one or more polypeptide chains.
iv. The amino acid residues are linked by repeating polypeptide bonds.
v. The adjacent polypeptide chains are linked by disulphide bonds.
vi. Most of the structural proteins which are in the form of fibres exhibitprimary structure
vii. The primary structure provides informtion on the number andproportion of different amino acids in a protein.
Primary structures of a large number of proteins have beendetermined.
eg. i. human insulin has 51 amino acids distributed in two poly peptidechains. A chain-31 amino acids, B chain-20 amino acids andthe polypeptides are linked by disulphide bridges.
ii. cytochrome C contains 104 amino acids.
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iii. human serum albumin contains 584 amino acids.
Primary structure is ultimately responsible for the native structureof the protein.
5.5.2 Secondary structure
The peptide chain thus formed assumes a two-dimentionalsecondary structure by way of folding or coiling consisting of a helicallycoiled, zig-zag linear or mixed form. It results from the steric relationshipbetween amino acids located relatively near to each other in the peptidechain. The linkages or bonds involved in the secondary structureformation are hydrogen bonds and disulphide bonds.
i. Hydrogen bond
These are weak, low energy non-covalent bonds sharing a singlehydrogen by two electronegative atoms such as O and N. Hydrogenbonds are formed in secondary structure by sharing H-atoms betweenoxygen of and nitrogen of of different peptide bonds.
C O ...........H N
The hydrogen bonds in secondary structure may form either anα-helix or β-pleated sheet structure.
ii. Disulphide bond
These are formed between two cysteine residues. They are strong,high energy covalent bonds.
Proteins exist in the two forms of secondary structure, α helix andβ pleated sheet.
5.5.2.1 α α α α α-Helix
A polypeptide chain forms regular helical coils called α-helix. Thesecoils are stabilized by hydrogen bonds between carbonyl oxygen of
C
O
N
H
(Hydrogen bond)
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first amino and amide N of fourth amino acid residues. Thus in α-helixintra chain hydrogen bonding is present. The α-helices can be eitherright handed or left handed. Left handed α-helix is less stable becauseof the steric interference between the carbonyl group and the sidechains. Only the right handed α-helix has been found in protein structure(Fig.5.5).
Fig. 5.5 ααααα-Helix structure
Each amino acid residue advances by 0.15 nm along the helix and3.6 amino acid residues are present in one complete turn. The distancebetween two equivalent points on turn is 0.54 nm and is called a pitch.
Small or uncharged amino acid residues such as alanine, leucineand phenyl alanine are often found in α-helix. More polar residuessuch as arginine, glutamate and serine may repel and destabilize α-helix. Proline is never found in α-helix.
Hair, nail, skin contain a group of proteins called keratins rich in α-helical structure.
5.5.2.2 βββββ-pleated sheet structure
A conformation called β pleated sheet structure is thus formedwhen hydrogen bonds are formed between the carbonyl oxygens and
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amide hydrogens of two or more adjacent extended polypeptide chains.Thus the hydrogen bonding in β pleated sheet structure is interchain.The structure is not absolutely planar but is slightly pleated due to thebond angles. The adjacent chains in β-pleated sheet structure are eitherparallel or antiparallel, (Fig.5.6) depending on whether the amino tocarbonyl peptide linkage of the chains runs in the same or oppositedirection.
NH
C
HN
C
NH C
NH
C
HN
C
NH
H2N
..............
Anti parallel Chains
C
HN
C
NH
C C
NH
C
HN
C
NH2
O ........
NH2
R
.........
...
O
R
RRR
O
O
R
O
R
O ..........HNNH
Parallel chains
CO
R
O
R
O
COOH
R
O
R
..............
O
R
O ..............
Fig. 5.6 βββββ-pleated sheet structure
In both parallel and antiparallel β-pleated sheet structures, theside chains are on opposite sides of the sheet. Generally glycine, serineand alanine are more common to form β-pleated sheet. Proline occursin β-pleated sheet although it tends to distrupt the sheets by producinglinks. Silk fibroin, a protein of silk worm is rich is β-pleated sheet.
5.5.3 Tertiary structure
The polypeptide chain with secondary structure may be furtherfolded, super-folded, twisted about itself forming many sizes. Such astructural confirmation is called tertiary structure. It is only one suchconfirmation which is biologically active and protein in this conformation
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is called as native protein. Thus the tertiary is constitued by stericrelationship between the amino acids located far apart but brought closerby folding (Fig. 5.7). The bonds responsible for interaction betweengroups of amino acids are as follows.
i. Hydrophobic interactions
Normally occur between nonpolar side chains of amino acids suchas alanine, leucine, methionine, isoleucine and phenyl alanine. Theyconstitute the major stabilzing forces for tertiary structure forminga compact three-dimentional structure.
ii. Hydrogen bonds
Normally formed by the polar side chains of the amino acids.
iii. Ionic or electrostatic interactions
The interaction occurs between oppostively charged polar sidechains of amino acids, such as basic and acidic amino acids.
iv. Vander -wall forces
Occurs between non polar side chains.
v. Disulphide bonds
These are S-S bonds formed between - SH groups of distantcysteine residues.
Fig. 5.7 Tertiary structure (eg. Myoglobin)
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5.5.4 Quarternary structure
Some proteins are made up of more than one polypeptide chainThese peptide chains held together by non-covalent interactions or bycovalent cross - links it is referred to as the quarternary structure. Theassembly is often called as an oligomer and each constituent peptidechain is called as a monomer or sub unit. The monomers of oligomericprotein can be identical or quite different in primary, secondary or tertiarystructure (Fig. 5.8).eg:
Proteins with 2 monomers (dimer) eg. Creatine phosphokinaseProteins with 4 monomers (tetramer) eg. Haemoglobin
Fig. 5.8 Quarternary sturcutre (eg. haemoglobin)
5.6 Biologically important proteins
i. Glutathione is a tripeptide containing glutamic acid, cysteine andglycine. It is present in erythrocytes and several other tissues. Itacts as a coenzyme and protects haemoglobin against oxidation.
ii. Insulin and glucagon are pancreatic hormones, involved in theregulation of glucose metabolism.
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iii. Angiotensin is a peptide which stimulates the release of certainhormones from adrenal gland.
iv. Collagen, is a connective tissue protein rich in proline and hydroxyproline.
5.6.1 Plasma proteins
Plasma consists of many proteins such as albumin, globulin andfibrinogen. Total protein of the plasma is about 6-8gm /100ml. Plasmaproteins comprise a major part of the solids of plasma. Albumin combinewith substances of low solubilities such as cholesterol, triacylglycerolto form more soluble complexes, which can be transported in the anaqueous environment of the body fluids.
Excercise
I. Choose the correct answer from the given four altenratives
a. Phenyl alanine is a
i. Aromatic amino acid ii. Aliphatic amino acid
iii. Dipeptide iv. Glycoprotein
b. Essential amino acids
i. are synthesized in the body
ii. are not synthesized in the body
iii. are not used for protein biosynthesis
iv. are unstable
c. The primary structure of proteins is associated with this
i. Amino acid sequence
ii. β-pleated sheet structure
iii. Conformation
iv. Relative position of subunits
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d. Protein denaturation results in
i. change of primary structure
ii. change of secondary structure.
iii. change of tertiary structure
iv. change in both secondary and tertiary structures.
e. The bonds responsible for the tertiary structure of proteins are
i. Hydrogen bonds
ii. Vander wall forces
iii. Disulphide bonds
iv. All the above.
II. Fill up the blanks
a. The simplest amino acid is -----------
b. All the amino acids exist in their ------------ form.
c. The functional group present in tryptophan is ------------
d. Guanidino group is present in the amino acid -------------
e. α helix nature of proteins tell about the ------------- structure ofproteins.
f. ---------------- amino acid is never found in α-helix
III. Say true or false
a. Proteins are not found in plants
b. Ornithine is a non-protein amino acid.
c. Glutamic acid has two carboxyl groups
d. Myoglobin can be analysed for its quaternary structure
e. A dipeptide has two peptide bonds.
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IV. Match the followings
a. Primary structure - Simplest amino acids
b. Glycine - Guanidino group
c. Zwitter ion - Amino acids sequence
d. Arginine - Quaternary structure
e. Hemoglobin - Tertiary structure
f. Myoglobin - Denaturing reagent
g. Urea - Isoelectric point
V. Give short answer for the followings
a. What is a peptide bond?
b. Give the D form of glycine.
c. Write the structure of Leucine.
d. How are proteins denatured?
e. Give the salient features of primary structure of a protein.
f. Name the any of two biologically important proteins with their
functions.
VI. Answer the followings
a. Give the classification of aminoacids.
b. Give the structure of aromatic amino-acids.
c. What are essential amino acids? Give examples.
d. Explain the secondary and tertiary structure of proteins.
e. What are the salient features of primary structure of proteins?
f. Write the reaction of an amino acid with ninhydrin reagent?
g. What is the action of Biuret reagent on proteins?